Report Project
Experiment 1. Isolation and characterization of proteolytic bacteriafrom the Sippewissett and “Dutch” sludge
Experiment 2. Isolation and characterization of methanogenic archaeafrom salt marsh, termite hindgut, and “Dutch” sludge
Submitted by
YAYA RUKAYADIDepartment ofBiology and Inter University Centerfor Biotechnology
Bogor Agricultural UniversityIndonesia
Microbial Diversity CourseMarine Biological LaboratoryWoods Hole - Massachusetts
Sunmier 1999
Acknowledgment
I thankful to the MBL for offering me this great opportunity, to Ed and Abigail fortheir support and encouragement. Specially thank very much to “Super Kurt” foreverything, to “my sister” Caroline that help me a lot in “methanogenic archaeaexperiment”, to Dawn for helpful in “proteolytic bacteria experiment”. Thank youso much to Tom, Joel, Scott, Rolf, Kalina, and Nell for everything. To all my friendsin the microbial diversity course : Joe, Tina, Jim, Eric, Brent, Kelvin, Allison,Tracy, Carry, Sherry, Donna, Jakob, Spencer, Yvone, Lesley, Jaque, Crist, Osnat,Barbara, and Lilliam thank and I love you....so much!
Yaya RukayadiJuly 29, 1999
Project 1.Isolation and characterization of proteolytic bacteria from the Sippewissett
and “Dutch sludge
Yaya Rukayadi
AbstractThe objective of this experiment was to isolate and characterize proteolytic bacteria fromenvironments; Sippewissett salt marsh and granular sludge from a UASB reactors.Proteolytic activity was determined for a total of 16 isolates and the three isolates (P1,P7, and UP-i) with the highest specific activity were characterized. The optimumtemperatures of the proteases made by P1, P7, and UP-i were 37°C, 25°C, and 50°C,respectively. The optimum pH of al of these proteases was approximately 7.5. Afteraddition of 5 mM EDTA, the specific activity of P1 was described by 18.39 %, 8.85 %(P7) and no activity was detected in the UP-i reaction. Also these enzymes seemed to beinhibited by the addition of PMSF. This result indicated that these enzymes containserine in its active site. 16S-rRNA genes fragments from the sixteen isolates wereamplified with eubacteria primers in the generation of sixteen 500 bp fragments. Thecomparative RFLP restriction enzymes confirmed that 7 of these 16 isolates can beclassified into three distinctive distribution patterns.
Project 2.Isolation and characterization of methanogenic archaea from the
Sippewissett, termite hind gut, and “Dutch” sludge
Yaya Rukayadi
AbstractThe objective of this study was to isolate and characterize methanogenic archaea fromthe Sippewissett salt marsh, termite hind gut, and “Dutch sludge. Mthanogenic archaeawere detected in cultures by production of methane. The samples from “Dutch” sludgeproduced the levels of methane, indicates that the sludge samples contained a largepopulation of methanogenic archaea. We also did a dilution series, and found that moremethane was produced in the 1:1010 dilution than the 1: dilution. Termite hind gutmicroorganism have also been shown to produce methane, and methanogenic archaeafrom these samples were grown on roll agar tubes and microscopically visualized. Inaddition, specimens from the primary enrichment of the sludge and termite hind gut wereexamined for methanogenic archaea by Fluorescent in situ hybridization (FISH).Specimens were hybridized with a rhodamin labeled archaea probe. Fluorescent cellswere seen in the primary enrichment of the sludge and termite hind gut of the examinedspecimens, which hybridized with the archaea probe. 16S-rDNA from the 8 isolates wereamplified using archaea primer and 3 PCR products (termite hind gut, sludge, and XF)were generated . The comparative RFLP analysis of the 16S-rDNA using HinPI and MspIrestriction enzymes confirmed that all isolates have distinctive distribution patterns. Thisresult indicated that the methanogenic archaea in the termite hind gut, Sippewissett (XF),and “Dutch” sludge are indeed different strains.
2
and sea water. The sample concentration of the suspension was adjusted to i04. 100 tl of
sample suspension was used to spread onto the plates. All cultures inoculated with sludge
were incubated at 37°C and Sippewissett cultures were inoculated at room temperature.
Extracellular proteinase-containing cell free supernatant. Cells were grown in liquid
medium with the same composition as skim milk solid medium used above. After a 24
hour incubation, the cells were centrifuged at 5000 rpm for 10 minutes. The supernatant
was their diluted 10 times usingNa2HPO4/NaH2PO4buffer at pH 7.0, and was used for
enzyme investigation.
Protease and protein assay. The proteolytic activity was measured according to method
of Bergmeyer and Grassi (1983) using 0.2% casein (Sigma) as the protein substrate, One
unit (U) of protease activity was defined as the amount of enzyme that yielded the
equivalent of 1 (mole tyrosine/minute under certain conditions. Protein concentration
was determined by the method suggested by Bradford (1976) with bovine serum albumin
fraction V (Merck) as a standard.
Optimum pH and temperature. The optimum temperature of the proteolytic activity
for each the strain was determined in 0.1M sodium phosphate buffer at pH 7. A shaking
waterbath was used for incubation in the temperature range of 18-55°C. The optimum
pH of the enzyme was also determined at optimum temperature in universal buffer and
activity was determined for pH values ranging from 5.56 to 10.5.
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Effect of protease inhibitors. Phenylmethylsulfonyl fluoride (PMSF) and EDTA in a
final concentration of 2 and 5 mM was added to cell free supematant and incubated at
room temperature (25°C) for 1 hour. The remaining protease activity was measured as
described previously. The protease activity without inhibitor was considered as 100%
activity.
DNA extraction and PCR amplification of the 16S rDNA. PrepMan Method (PE
Applied Biosystems a division of Perkin-Elmer) provided during the course was used to
extract DNA from proteolytic bacteria. MicroSeq’ 500 165 rDNA Bacterial Sequencing
Kit (PE Applied Biosystems a division of Perkin-Elmer) was used for PCR amplification
of DNA extracted from proteolytic bacteria. The amplification was carried out in 50 .tl
reaction volume: 25 il PCR Master Mix and 25 jl diluted genomic DNA extraction. The
PCR temperature profile was as follows: 95°C for 10 mm, 30 cycles of (95°C for 30 sec,
60°C for 30 sec, 72°C for 45 sec), the amplification time of each cycle was extended for 5
sec. Amplified DNA was examined by horizontal electrophoresis in 1.25% agarose with
5 .d aliquots of the PCR product.
Restriction fragment length polymorphism (RFLP). Aliquots of PCR products were
mixed with the restriction endonucleases HinPI and MspI. Reaction mixtures of 20 p1
containing: 10 p1 PCR product, 2 p1 restriction buffer Neb2 (New England Biolab), 8.6 p1
dH2O and 0.2 each of restriction enzyme. Restricted DNA was analysed by horizontal
electrophoresis in a 2 % agarose. The resulting band patterns were used to distinguish
different clusters of bacteria.
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Results and Discussion
Isolation and proteolytic production. Figure 1 shows the presence of clearing zones
surrounding colonies grown on the selective medium. A total of 16 isolates were
analysed for their proteolytic activity and the three isolates (P1, P7, and UP-i) with the
highest apecipic activity were characterized. Proteolitic activity exhibited by these
isolates is shown in Table 1. In addition microscopic observation of the two isolates (UP
1 and FVA) can be seen in Figure 2.
Effect of temperature and pH. Figure 3 and 4 show the effect of temperature and pH on
proteolytic activity. The optimum temperatures of the proteases made by P1, P7, and UP-
1 were 37°C, 25°C and 50°C respectively. The optimum pH of the proteases was
approximately 7.5.
Effect of protease inhibitors. For classification of these proteases, its activity was
measured in the presence of specific protease inhibitors. Figure 5 indicated that these
enzymes are metalloenzymes since EDTA at concentration of 5 mM almost totally
inhibited the activity. After addition of EDTA, the specific activity of Pi was only 18.39
% (P1), 8.85% (P7) and no activity was detected in the UP-i reaction. Also, we found
that these enzymes seem to be inhibited by the addition of PMSF. The activity of P1
decreased by 67.04%, 76.21 for P7, and 78.07% for UP-i after one hour incubation with
5 mM inhibitor. This result indicated that the enzymes contains serine in its active site.
5
DNA extraction, PCR amplification of the 16S rDNA, and Restriction fragment
length polymorphism (RFLP). 16S-rDNA genes from the sixteen isolates have been
amplifield resulting in the generate on of sixteen 500 bp fragments (Figure 6). The
comparativeRFLP analysis of the 16S-rDNA using Hinfi and MspI restrictions enzymes
confirmed that 7 of the 16 isolates can be classified into three distinctive distribution
patterns (Figure 7). Group I includes only isolate P2. P4,P7, P9, and UP-i isolates can be
found in group II and , PG into group ifi category.
Suggested References
Bergmeyer, H. U & m. grassl. 1983. Methods of enzymes analysis. Vol. 2. VerlagChemie, Weinheim.
Bradford, M. M, 1976. A rapid and sensitive method for quantitation of microgramquantities of protein dye binding. Analytical Biochemistry, 72, 284-294.
Eggen, R., A. Geerling, J. Watts & W. M de Vos, 1990, Characterization of pyrolysin, ahyperthermoactive serine protease from the archaebacterium Pyrococcusfuriosus,FEMS , 71, 17-20.
Fusek, M., Lin, X-L & Tang, J., 1990, Enzyme properties of thermopsin, J. Bio.Chem.,265, 1496-1501
Klingerberg, M., B. Galunsky, C. Sjoholm, V. Kasche & G. Antranikian, 1995,Purification and properties of a highly thermostable, sodium dodecyl sulfate-resistant and stereospecific proteinase from extremely thermophilic archaeonThermococcus stetteri, App. Env. Microb, Aug, p. 3098-3 104.
Matsuzawa, H., Hamaoki, M & Ohta, T., 1983, Production of thermophilic protease(aqualysin I and II) by Thermus aquaticus YT-1, an extreme thermophile, Agric.Biol. Chem., 47, (1), 25-28
Morihara, K and Oda, K., 1992, In Microbial degradation of natural products, (ed.Winkelmann, G.), VCH, Weinheim, pp. 293-364,
Tsuchiya, K., Y. Nakamura, H. Sakashita & T. Kimura, i992, Purification andcharacterization of a thermostable alkaline protease from alkalophilicThermoactinomyces sp. HS682, Biosci. Biotech. Biochem, 56 (2). 246-250.
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Table 1.
No. Isolates Proteolytic activity (Units! mgprotein)
1 P1 (VFA sludge) 13.5902 P2 (XF-Sippewissett) 7.3783 P3 (Aviko sludge) 5.3644 P4 (UP-2 Sippewissett) 12.1255 P5 (C1-Sippewissett) 3.8276 P6 (C1-Sippewissett) 6.2397 P7 (C1-Sippewissett) 60.0708 P8 (HF-Sippewissett) 18.4709 P9 (HF-Sippewissett) 3.55010 P10 (C1-sippewissett) 5.94511 PD (HF-Sippewissett) 11.41612 PE (C1-Sippewissett) 13.45513 PF (Aviko sludge) 4.63814 PG (C1-Sippewissett) 4.03515 PH (VFA-Sludge) 4.46116 UP-i (Sippewissett) 14.925
4.
Figure 1
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Experiment 2. Isolation and characterization methanogenic archaea from theSippewissett salt marsh, termite hind gut, and “Dutch” sludge
Introduction
The methanogenic archaea produced large quantities of methane as the major
product of their energy metabolism and are strictly anaerobic. Methanogenesis is the
terminal step in the carbon flow in many anaerobic habitats. Biogenic methane
formation occurs in a wide variety of environments such as, ruminants, termites,
cockroaches, mammals, lakes, wetland, sludge, landfills, oceans, tundra fields and
human-made waste water treatment plants and other systems for bioremediation. The
methanogenic archaea produce methane primaily fromH2-C02and in some cases,
from formate, acetate, methanol or methylamine.
The main goals of this study were to isolate and characterize methanogenic
archaea from the Sippewissett salt marsh, termite, and granular sludge from a UASB
reactors from The Netherland.
Materials and Methods
Primary enrichment. Enrichment cultures for each sample were maintained in 60-ml
serum bottles containing liquid medium. Granular sludge from UASB reactors (The
Netherland), termite hind gut, and soil from both fertilized and unfertilized plots from
Sippewissett were examined. The granular sludge and termite hind gut samples were
first diluted in phosphate buffer, and the Sippewissett samples were diluted in sea
water. Concentration of all samples was adjusted to iO. 100 j.il of sample suspension
2
was used to inoculate all of the bottles. All cultures were incubated in the dark, sludge
was incubated at 37°C, termite hind gut cultures at 30°C, and Sippewissett cultures
were incubated at 22°C. Before inoculation, the bottles contained 18 ml standard
medium, gassed with either nitrogen orH2-C02(80:20) and pressurized to 0.5 atm.
Methanol was used as carbon source for Sippewissett and sludge cultures, and H2-
CO2 was carbon source for termite hind gut cultures..
Isolation of methanogenic archaea. Roll agar tubes (3%) were used to isolated
methanogenic archaea. The roll agar tubes were inoculated aseptically under nitrogen
orH2-C02and then were gassed, pressurized, and inoculated as described above.
Secondary enrichment. A single colony from the roll agar tubes, was transferred
into liquid medium aseptically under nitrogen orH2-C02and was then gassed,
pressurized, and inoculated as described above.
Methane analysis. Gas chromatography (GC) was used to determine methane
production in the primary and secondary enrichment cultures and roll agar tubes
cultures. The gas chromatograph (Varian 3800) was fitted with a CP-Poroplot U
column (Chrompach/Varian) and a flame ionization detector (FID). The
chromatographic conditions were: 50°C running temperature and 80°C detection
temperature. A standard of 1 % of methane in air was used to calibrate the gas
chromatograph.
3
Microscopic observation. A Zeiss microscope was used to determined whether
coenzyme-420 which is found in methanogenes could e detected in net mounts made
from the enrichment cultures. The microscope was arranged so that this coenzyme
could be observed by epifluorescence microscopy. In addition, , the microscope was
attached to a video camera, a monitor and a computer to enable image capture and
processing.
Fluorescent in situ hybridization (FISH). A rhodamine labeled archaea probe was
used to detect methanogenic archaea in enrichments, and the termite hind gut.
Treatment of specimens and hybridization reaction protocols were carried out as
described in the workshop manual provided by Scott Davson.
DNA extraction and PCR amplification of the 16S rDNA. PrepMan Method (PE
Applied Biosystems a division of Perkin-Elmer) provided during the course was used
to extract DNA from both secondary enrichment and a single colony selected from
roll agar tubes containing methanogenic archaea. Universal archae primers, 21F
forward (position 21) 5’-TTCCGGTTGATCCYGCCGGA-3’ and 915AR reverse
(position 915) 5’-GTGCTCCCCCGCCAATTCCT-3’ were used for PCR
amplipication of DNA extracted from the secondary enrichment and the single colony
in roll agar tube. The amplification was carried out in a 50 j.tl reaction volume: 1 jii
of template DNA with 49 jil of polymerase reaction mixture. Each reaction mixture
4
received one bead containing the Tag polymerase. The PCR temperature profile was
as follows: 95°C for 10 mm, 30 cycles of (95°C for 30 sec, 60°C for 30 sec, 72°C for
45 sec), the amplification time of each cycle was extended for 5 sec. Amplified DNA
was examined by horizontal electrophoresis in 1.25% agarose with 5 j.tl aliquots of
the PCR product.
Restriction fragment length polymorphism (RFLP). Aliquots of PCR products
were mixed with the restriction endonucleases HinPI and MspI. Reaction mixtures of
20 p.1 containing: 10 p.1 PCR product, 2 p.1 restriction buffer Neb2 (New England
Biolab), 8.6 p.1 dH2O and 0.2 each of restriction enzyme. Restricted DNA was
analyzed by horizontal electrophoresis in a 2 % agarose. The resulting band patterns
were used to distinguish between different species of bacteria.
Results and Discussion
Methane production. Production of methane was used as indicator of methanogenic
activity. Methane production was detected in the primary and secondary enrichments
and roll agar tubes (Table 1).
Table 1. Methane production from the primary and secondary enrichments and rollagar tubes
Sample Methane (%)Week 1 Week 2 Week 3
“Dutch” sludge (primary enrichment-roll agar tube)1. Avikoa. high dilution 1.69 59.46 448.28
5
b. low dilution ND 0.13 0.09
2. CSMa. high dilution 0.61 7.98 120.81b.low dilution ND 0.09 0.16
3.VFAa. high dilution 76.80 556.77 365.04b. low dilution 0.61 6.66 6.74
“Dutch” sludge (secondary enrichment-liquidmedium)1.Aviko 0.04 0.042. CSM 0.04 0.043.VFA 0.46 0.04
Sippewissett (primary enrichment-liquid medium)C 1.03 0.02UP 0.43 0.04HF 0.19 0.02XF 3.96 ND
Sippewissett (primary enrichment-roll agar tube)C 0.58 2.34UP 0.08 2.45HF 1.17 72.44XF 0.92 1.55
Termite hindgut (primary enrichment-roll agar 0.07 2.04tube)ND : non-detectionC : control or unfertilizedUP : fertilized using urea and phosphatHF: high ferlilizedXF: extra fertilizedHigh dilution (1: 1O’°)Low dilution (1: 1O)
Table 1 shows that the samples from “Dutch” sludge produced the highest
levels of methane, suggesting that the sludge samples contained the largest
concentrations of methanogenic archaea. We also found that methanogenic archaea
6
activity in high dilution was higher than low dilution. This low value of methane
found in the high dilution might be explaned by competition between methanogenic
archaea with an other microanaerobic organism. Termite hindgut microorganisms
have also been shown to produce methane, and methanogenic archaea have been
visualized from some clonies in roll agar tube.
Isolation and microscopic observation. Methane production was detectable in the
roll agar tubes and fluorescence was observed. This result indicates that
methanogenic archaea were sucessfully isolated. Methanogenic archaea from “Dutch”
sludge can be seen in Figure 1.
Fluorescent in situ hybridization (FISH). Specimens from primary enrichment of
sludge and termite hind gut were examined for methanogenic archaea by Fluorescent
in situ hybridization (FISH). Specimens were hybridized with a rhodamin labeled
archaea probe. Cells that hybridized with the archaea probe were seen in the primary
enrichment of sludge and the termite hind gut. The result of FJSH can be seen in
Figure 2.
DNA extraction, PCR amplification of the 16S rDNA, and Restriction fragment
length polymorphism (RFLP). 16S-rDNA squences from the 8 isolates have been
amplifield using archaeal primers and 3 PCR products were generated (Figure 3). The
comparative RFLP analysis of the 16S-rDNA using HinPI and MspI restriction
7
enzymes confirmed that all isolates can be classified into different distinctive
distribution patterns (Figure 4). This result indicates that the methanogenic archaea in
the termite hind gut, Sippewissett, and “Dutch” sludge are different strains.
Suggested References
Cheesman, P., A. Toms-Wood & R.S. Wolfe. 1972. Isolation and properties of a
fluorescent compound, Factor420,from Methanobacterium strain M.o.H.
Miller, T.L. and M.J. Wolin. 1985. Methanosphaera stadtmanae gen. Nov., sp. Nov.
a species that forms methane by reducing methanol with hydrogen. Arch.
Microbiol. 141, 116-122.
Thauer, R., K. 1998. Biochemistry of methanogenesis: a tribute to Marjory
Stephenson. Microbiology, 144, 2377-2406.
Messer, A., C. & M. J. Lee. 1989. Effect of chemical treatment on methane emission
by the hindgut microbiota in the termite Zootermopsis angusticollis. Microb.
Ecol., 18,275-284.
8
A
B
Fluorescent in situ hybridization (FISH)(Rhodamin labeled archaea)
A. Aviko sludge enrichment
B. Termite hind gut
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